Synergizing Exchangeable Fluorophore Labels for Multitarget STED Microscopy

被引:22
作者
Glogger, Marius [1 ]
Wang, Dongni [1 ]
Kompa, Julian [2 ]
Balakrishnan, Ashwin [1 ]
Hiblot, Julien [2 ]
Barth, Hans-Dieter [1 ]
Johnsson, Kai [2 ,3 ]
Heilemann, Mike [1 ]
机构
[1] Goethe Univ Frankfurt, Inst Phys & Theoret Chem, D-60438 Frankfurt, Germany
[2] Max Planck Inst Med Res, Dept Chem Biol, D-69120 Heidelberg, Germany
[3] EEcole Polytech Fed Lausanne EPFL, Inst Chem Sci & Engn ISIC, CH-1015 Lausanne, Switzerland
关键词
Super-resolution microscopy; DNA-PAINT; STED; exchangeable fluorophores; multicolor imaging; live-cell imaging; Halo-Tag; SUPERRESOLUTION MICROSCOPY; BINDING; CELLS;
D O I
10.1021/acsnano.2c07212
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
Investigating the interplay of cellular proteins with optical microscopy requires multitarget labeling. Spectral multiplexing using high-affinity or covalent labels is limited in the number of fluorophores that can be discriminated in a single imaging experiment. Advanced microscopy methods such as STED microscopy additionally demand balanced excitation, depletion, and emission wavelengths for all fluorophores, further reducing multiplexing capabilities. Noncovalent, weak-affinity labels bypass this "spectral barrier " through label exchange and sequential imaging of different targets. Here, we combine exchangeable HaloTag ligands, weak-affinity DNA hybridization, and hydrophophic and protein-peptide interactions to increase labeling flexibility and demonstrate six-target STED microscopy in single cells. We further show that exchangeable labels reduce photobleaching as well as facilitate long acquisition times and multicolor live-cell and high-fidelity 3D STED microscopy. The synergy of different types of exchangeable labels increases the multiplexing capabilities in fluorescence microscopy, and by that, the information content of microscopy images.
引用
收藏
页码:17991 / 17997
页数:7
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